I-TIANcombi DNA Lyse & Det PCR Kit

Ukuhlanzwa okusheshayo kwe-DNA kusuka ezintweni ezahlukahlukene zokutholwa kwe-PCR.

I-TIANcombi DNA Lyse & Det PCR Kit isebenzisa idizayini eyingqayizivele yokufaka okubandakanya wonke ama-reagents wokulungiselela i-genomic DNA ngokushesha nokwandisa i-PCR. Kusebenza ekuhlanzweni kwe-DNA yesinyathelo esisodwa kusuka kumasampula ahlukahlukene (izicubu zezitshalo, imbewu, izicubu zezilwane, igazi, imvubelo kanye namagciwane) kanye nokukhuliswa nokutholwa kwePCR okulandelayo. Amaphrotheni, i-RNA nokunye ukususwa kwe-metabolites yesibili, ukukhishwa kwe-organic solvent kanye nezinyathelo zokuthambisa ze-ethanol azidingeki kuyo yonke inqubo yokuhlanzwa, okwenza umsebenzi ube lula futhi usheshe. Ikhwalithi yomkhiqizo izinzile futhi inokwethenjelwa.

I-2 × Det PCR MasterMix enikezwe yile khithi iyi-reagent ehambisanayo kakhulu ye-PCR ekwazi ukukhulisa kahle nangokuqondile i-DNA ngaphandle kwesidingo sokususa ukungcola njengamaprotheni. Le reagent iqukethe i-Taq DNA polymerase, i-dNTPs, i-MgCl₂, i-buffer, kanye ne-enhancer, optimizer kanye ne-stabilizer yokuphendula kwe-PCR. Ukusetshenziswa kwe-reagent kwenza ukusabela kwe-PCR kusheshe, kube lula, kuzwele, kucaciswe futhi kuzinze. Ngakho-ke, le kit ikulungele ikakhulukazi ukuhlolwa okuphezulu.

Ikati. Cha	Ukupakisha Usayizi
4992527	20 ×l × 50 rxn
4992528	20 µl × 200 rxn

Thumela i-imeyili kithi

Imininingwane yomkhiqizo

Isibonelo sokuhlola

Imibuzo evame ukubuzwa

Amathegi womkhiqizo

Izici

■ Ilula futhi iyashesha: I-DNA yezicubu ezahlukahlukene ingakhishwa ngemizuzu engu-5 ngaphandle kwesidingo sokugaya i-nitrogen engamanzi.
■ Izicelo ezibanzi: Kusetshenziswa amaqabunga ezitshalo, imbewu, izicubu zezilwane, amasampula egazi (igazi elisha, i-anticoagulation, amahlule egazi, amabala egazi omisiwe, njll.), Imvubelo namagciwane.
■ Ukuhambisana okunamandla: I-reagent ye-PCR ilungele ukukhuliswa kwe-DNA ekhishwe emithonjeni ehlukahlukene yesampula.

Izicelo

■ Ukutholwa kwe-Gene: Ukukhetha okufanele ukutholwa kwezakhi zofuzo ezinkulu.

Amanothi abalulekile

■ Kumasampuli aqukethe izinga eliphezulu lama-phenols, njengamaqabunga kakotini, inani lesampula lokufaka kufanele libe ngaphansi kuka-0.4 mg, ngaphandle kwalokho ukusabela kwe-PCR kuzothinteka.

Yonke imikhiqizo ingenziwa ngezifiso i-ODM / OEM. Ngemininingwane,sicela uchofoze i-Customized Service (ODM / OEM)

Langaphambilini I-GMO Crop Extraction & Kit Yokukhulisa

Olandelayo: Igazi Direct PCR Kit

	I-DNA ikhishwe ku-5 mg wamaqabunga nembewu yommbila, ukolweni, ilayisi, ubhontshisi wesoyoni nokotini, ngokulandelana. I-DNA yandiswa yi-PCR isebenzisa iziqalo ezithile. I-6 μl DNA kusuka kumakholomu angama-20 μl alayishwe kulayini ngamunye. 1: Ukulawulwa okuhle kwe-genome; 2: shiya amasampula; 3: amasampula wembewu; 4: I-NTC; 5: ama-primer ama-D2000
	M: Umaka we-TIANGEN D2000; 1: Ukulawula okuhle; 2-7: Inani lamachashazi egazi omisiwe ephepheni lokuhlunga liyi-1-6 ngokulandelana; 8: Ukulawulwa okungekuhle. I-puncher engu-3 mm isetshenziselwe ukuthatha izindawo ezomile zegazi ezivela ephepheni lokuhlunga njengezinto zokuhlolwa kokukhishwa. I-6 μl DNA kusuka kumakholomu angama-20 μl alayishwe kulayini ngamunye.
	M: Umaka we-TIANGEN D2000; 1: Ukulawulwa okuhle (i-genomic DNA isetshenziswe njengethempulethi); 2-7: Inani legazi elengeziwe liyi-10 μl, 20 μl, 30 μl, 40 μl, 50 μl ne-60 μl, ngokulandelana; 8-13: Inani legazi elengeziwe liyi-10 μl, 20 μl, 30 μl, 40 μl, 50 μl ne-60 μl, ngokulandelana; 14: I-NTC. I-6 μl DNA evela kuma-eluents angama-20 μl alayishwe ku-gel agarose.

Q: Awekho amabhendi wokukhulisa

Isifanekiso se-A-1

■ Ithempulethi iqukethe ukungcola kwamaprotheni noma ama-Taq inhibitors, njll. - —Purify DNA template, susa ukungcola kwamaprotheni noma ukhiphe i-DNA template ngamakhithi okuzihlanza.

■ Ukwehlukaniswa kwethempulethi akuphelele ——Kwandisa ngokufanele ukushisa kwama-denaturation futhi kwandise isikhathi se-denaturation.

■ Ukuwohloka kwesifanekiso ——Lungisa kabusha ithempulethi.

I-A-2 Primer

■ Izinga eliphansi lama-primers ——Re-synthesize the primer.

■ Ukuwohloka kwe-Primer ——Faka ama-primer primer aphezulu abe yivolumu encane yokulondolozwa. Gwema ukubanda okuningi nokuncibilikisa noma ukugcina isikhathi eside u-4 ° C.

■ Idizayini engalungile yama-primers (isb. Ubude be-primer abwenele, i-dimer eyakhiwe phakathi kwama-primers, njll.) -Redesign primers (gwema ukwakheka kwe-primer dimer nesakhiwo sesibili)

I-A-3 Mg²⁺ukuhlushwa

■ Mg²⁺ ukuminyana kuphansi kakhulu —— Khulisa ngokufanele uMg²⁺ukuhlushwa: Lungiselela iMg²⁺ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile²⁺ ukugxila kuthempulethi ngayinye nakuqala.

Ukushisa kwe-A-4 Annealing

The Ukushisa okuphezulu kokunciphiswa komthelela kuthinta ukubopha kwe-primer ne-template. - - Nciphisa ukushisa okunciphisayo futhi wenze ngcono isimo nge-gradient ka-2 ° C.

Isikhathi se-A-5 Sesandiso

■ Isikhathi esifushane sokunweba — - Khulisa isikhathi sokunweba.

Umbuzo: Ukuthi kunamanga

I-Phenomena: Amasampula amabi nawo akhombisa amabhendi wokulandelana okuqondiwe.

Ukungcola kwe-A-1 kwe-PCR

■ Ukungcola kwesiphambeko sokulandelana okuqondiwe noma imikhiqizo yokukhulisa amandla ——Nakekela ukuthi ungafaki isampuli ngesampula equkethe ukulandelana kwethagethi kusampula engeyinhle noma uchithe iphume kushubhu le-centrifuge. Ama-reagents noma okokusebenza kufanele kwenziwe ngokuzenzakalela ukuqeda ama-nucleic acid akhona, futhi ubukhona bokungcola kufanele kunqunywe ngokuhlolwa kokulawulwa okungalungile.

■ Ukungcola okuyisenzo ——Faka ama-reagents bese uwagcina lapho kushisa okuncane.

I-A-2 Primer

■ Mg²⁺ ukuminyana kuphansi kakhulu —— Khulisa ngokufanele uMg²⁺ ukuhlushwa: Lungiselela iMg²⁺ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile²⁺ ukugxila kuthempulethi ngayinye nakuqala.

■ Idizayini yokuqala engafanele, nokulandelana kwempokophelo kune-homology ngokulandelana okungeyona eyenhloso. ——Kwakha kabusha ama-primers.

Q: Ukukhulisa okungacacisiwe

I-Phenomena: Amabhendi wokukhulisa we-PCR awahambelani nosayizi olindelekile, kungaba mikhulu noma mincane, noma kwesinye isikhathi womabili amabhendi okukhulisa kanye namaqembu wokukhulisa angaqondile.

I-A-1 Primer

■ Ukucaciswa okungafanelekile kokuqala

——Kwakha kabusha isiqalo.

■ Ukuhlungwa kwe-primer kuphakeme kakhulu — -Kwandisa ngokufanele ukushisa kwe-denaturation futhi kwandise isikhathi se-denaturation.

I-A-2 Mg²⁺ ukuhlushwa

■ UMg²⁺ ukuminyana kuphakeme kakhulu —— Nciphisa kahle ukuhlushwa kwe-Mg2 +: Lungiselela iMg²⁺ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile²⁺ ukugxila kuthempulethi ngayinye nakuqala.

I-A-3 Thermostable polymerase

■ Inani le-enzyme eyeqile - - Nciphisa inani le-enzyme ngokufanele ngezikhathi ezithile zika-0.5 U.

Ukushisa kwe-A-4 Annealing

■ Izinga lokushisa elinciphisayo liphansi kakhulu ——Kwandisa ngokufanele ithempelesha yokuncisha noma ukusebenzisa indlela yokuncisha izigaba ezimbili

Imijikelezo ye-A-5 PCR

■ Imijikelezo eminingi kakhulu ye-PCR —— Nciphisa inani lemijikelezo ye-PCR.

Q: Ama-Patchy noma ama-smear bands

I-A-1 Primer—— Okucacile okungekuhle—— Yakha kabusha i-primer, shintsha ukuma nobude be-primer ukuthuthukisa ukucaciswa kwayo; noma wenze i-PCR ehlanganisiwe.

I-A-2 Template DNA

——Isifanekiso asihlanzekile —Hlanza ithempulethi noma ukhiphe i-DNA enezikhwama zokuhlanzwa.

I-A-3 Mg²⁺ ukuhlushwa

- —Mg²⁺ ukugxilisa ingqondo kuphakeme kakhulu ——Ukunciphisa kahle uMg²⁺ ukuhlushwa: Lungiselela iMg²⁺ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile²⁺ ukugxila kuthempulethi ngayinye nakuqala.

I-A-4 dNTP

—— Ukuhlungwa kwama-dNTP kuphakeme kakhulu —— Nciphisa ukuminyana kwe-dNTP ngokufanele

Ukushisa kwe-A-5 Annealing

——Ukushisa okuncishisayo okuphansi impela —— Kukhuphula kahle ukushisa okuncishisayo

Imijikelezo engu-A-6

—Imijikelezo eminingi kakhulu —— Yandisa inani lomjikelezo

Q: Mangaki ithempulethi ye-DNA okufanele ingezwe ku-50 μl system reaction reaction?

Q: Ungazikhulisa kanjani izingcezu ezinde?

Isinyathelo sokuqala ukukhetha i-polymerase efanelekile. I-Taq polymerase ejwayelekile ayikwazi ukufundwa ngenxa yokuntuleka komsebenzi we-3'-5 'wokuxolelwa, futhi ukungafani kahle kuzonciphisa kakhulu ukusebenza kwezingcezu. Ngakho-ke, i-Taq polymerase ejwayelekile ayikwazi ukukhulisa ngempumelelo izingcezu ezihlosiwe ezinkulu kune-5 kb. I-Taq polymerase enokuguqulwa okukhethekile noma okunye ukuthembeka okuphezulu kwe-polymerase kufanele kukhethwe ukuthuthukisa ukusebenza kahle kokunwetshwa nokuhlangabezana nezidingo zokukhulisa isiqeshana eside. Ngaphezu kwalokho, ukukhuliswa kwezingcezu ezinde kudinga nokulungiswa okuhambisanayo komklamo wokuqala, isikhathi sokudlulisa isikhathi, isikhathi eseluliwe, i-pH yesikhondlakhondla, njll. Ngokuvamile, ama-primers ane-18-24 bp angaholela esivunweni esingcono. Ukuvikela ukulimala kwethempulethi, isikhathi sokudonswa kwenani elingu-94 ° C kufanele sehliswe lifike kumasekhondi angama-30 noma ngaphansi ngomjikelezo ngamunye, nesikhathi sokukhuphuka kwamazinga okushisa siye ku-94 ° C ngaphambi kokukhulisa amandla kufanele kube ngaphansi kweminithi elilodwa. Ngaphezu kwalokho, ukusetha izinga lokushisa lokunwebeka cishe ku-68 ° C nokuklama isikhathi sesandiso ngokuya ngesilinganiso se-1 kb / min kungaqinisekisa ukukhuliswa okusebenzayo kwezingcezu ezinde.

Q: Ungakuthuthukisa kanjani ukwethembeka kokukhulisa kwe-PCR?

Izinga lephutha lokukhulisa i-PCR lingehliswa ngokusebenzisa ama-polymerase e-DNA ahlukahlukene ngokuthembeka okuphezulu. Kuwo wonke ama-polymerase eTaq DNA atholakele kuze kube manje, i-Pfu enzyme inezinga lephutha eliphansi kakhulu nokuthembeka okuphezulu (bheka ithebula elihlanganisiwe). Ngaphezu kokukhethwa kwe-enzyme, abacwaningi bangaqhubeka banciphise izinga lokuguqulwa kwe-PCR ngokwenza ngcono izimo zokuphendula, kufaka phakathi ukwakheka kwe-buffer, ukuminyana kwe-polymerase esetshenziswayo nokwandisa inombolo yomjikelezo we-PCR.

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